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首页> 外文期刊>European Biophysics Journal >Matchout deuterium labelling of proteins for small-angle neutron scattering studies using prokaryotic and eukaryotic expression systems and high cell-density cultures
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Matchout deuterium labelling of proteins for small-angle neutron scattering studies using prokaryotic and eukaryotic expression systems and high cell-density cultures

机译:使用原核和真核表达系统和高细胞密度培养的小角中子散射研究蛋白质蛋白质蛋白质标记

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摘要

Small-angle neutron scattering (SANS) is a powerful technique for the characterisation of macromolecular structures and interactions. Its main advantage over other solution state approaches is the ability to use D2O/H2O solvent contrast variation to selectively match out specific parts of a multi-component system. While proteins, nucleic acids, and lipids are readily distinguished in this way, it is not possible to locate different parts of a protein-protein system without the introduction of additional contrast by selective deuteration. Here, we describe new methods by which 'matchout labelled' proteins can be produced using Escherichia coli and Pichia pastoris expression systems in high cell-density cultures. The method is designed to produce protein that has a scattering length density that is very close to that of 100% D2O, providing clear contrast when used with hydrogenated partner proteins in a complex. This allows the production of a single sample system for which SANS measurements at different solvent contrasts can be used to distinguish and model the hydrogenated component, the deuterated component, and the whole complex. The approach, which has significant cost advantages, has been extensively tested for both types of expression system.
机译:小角度散射(SAN)是一种强大的技术,用于表征大分子结构和相互作用。其主要优点在于其他解决方案状态方法是能够使用D2O / H2O溶剂对比度变化来选择性地匹配多组分系统的特定部分。虽然蛋白质,核酸和脂质以这种方式容易地区分,但不可能定位蛋白质 - 蛋白质系统的不同部位,而不会通过选择性氘引入额外的对比度。在这里,我们描述了通过在高细胞密度培养物中使用大肠杆菌和Pichia牧场表达系统来生产“匹配标记的”蛋白质的新方法。该方法设计成产生具有非常接近100%D2O的散射长度密度的蛋白质,当与复合物中的氢化合作蛋白一起使用时,提供清晰的对比度。这允许生产不同溶剂对比度的SAN测量的单个样品系统可用于区分和模拟氢化组分,氘代组分和整个复合物。具有显着成本优势的方法已广泛测试两种类型的表达系统。

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